Ascorbic acid can promote the generation and expansion of neuroepithelial-like stem cells derived from hiPS/ES cells under chemically defined conditions through promoting collagen synthesis

Rui Bai; Yun Chang; Amina Saleem; Fujian Wu; Lei Tian; Siyao Zhang; Ya'nan Li; Shuhong Ma; Tao Dong; Tianwei Guo; Youxu Jiang; Yi You; Wen-Jing Lu; Hong Feng Jiang; Feng Lan

doi:10.1186/s13287-020-02115-6

Ascorbic acid can promote the generation and expansion of neuroepithelial-like stem cells derived from hiPS/ES cells under chemically defined conditions through promoting collagen synthesis

Stem Cell Res Ther. 2021 Jan 9;12(1):48. doi: 10.1186/s13287-020-02115-6.

Authors

Rui Bai^{1

2}, Yun Chang^{1

2}, Amina Saleem¹, Fujian Wu^{1

2}, Lei Tian³, Siyao Zhang^{1

2}, Ya'nan Li^{1

2}, Shuhong Ma^{1

2}, Tao Dong^{1

2}, Tianwei Guo^{1

2}, Youxu Jiang^{1

2}, Yi You^{4

5}, Wen-Jing Lu^{1

2}, Hong Feng Jiang^{6

7

8}, Feng Lan^{9

10

11

12}

Affiliations

¹ Beijing Laboratory for Cardiovascular Precision Medicine, MOE Key Laboratory of Medical Engineering for Cardiovascular Diseases, MOE Key Laboratory of Remodeling-Related Cardiovascular Disease, Beijing Collaborative Innovation Center for Cardiovascular Disorders, Anzhen Hospital, Capital Medical University, Beijing, 100029, China.
² Beijing Institute of Heart, Lung and Blood Vessel Diseases, Beijing, 100029, China.
³ Key Laboratory of Chinese Internal Medicine of Ministry of Education and Beijing, Dongzhimen Hospital Affiliated to Beijing University of Chinese Medicine, Beijing, China.
⁴ Center for Clinical Translation and Innovation, Peking University Shenzhen Graduate School, Shenzhen, 518055, China.
⁵ Shenzhen Bay Laboratory, Shenzhen, 518055, China.
⁶ Beijing Laboratory for Cardiovascular Precision Medicine, MOE Key Laboratory of Medical Engineering for Cardiovascular Diseases, MOE Key Laboratory of Remodeling-Related Cardiovascular Disease, Beijing Collaborative Innovation Center for Cardiovascular Disorders, Anzhen Hospital, Capital Medical University, Beijing, 100029, China. hfjiang@ccmu.edu.cn.
⁷ Beijing Institute of Heart, Lung and Blood Vessel Diseases, Beijing, 100029, China. hfjiang@ccmu.edu.cn.
⁸ Beijing Anzhen Hospital, Research Institute Building, Room 323, 2 Anzhen Road, Chaoyang District, Beijing, 100029, China. hfjiang@ccmu.edu.cn.
⁹ Beijing Laboratory for Cardiovascular Precision Medicine, MOE Key Laboratory of Medical Engineering for Cardiovascular Diseases, MOE Key Laboratory of Remodeling-Related Cardiovascular Disease, Beijing Collaborative Innovation Center for Cardiovascular Disorders, Anzhen Hospital, Capital Medical University, Beijing, 100029, China. fenglan@ccmu.edu.cn.
¹⁰ Beijing Institute of Heart, Lung and Blood Vessel Diseases, Beijing, 100029, China. fenglan@ccmu.edu.cn.
¹¹ State Key Laboratory of Cardiovascular Disease, National Center for Cardiovascular Diseases, Fuwai Hospital, Chinese Academy of Medical Sciences and Peking Union Medical College, Beijing, China. fenglan@ccmu.edu.cn.
¹² Beijing Anzhen Hospital, Research Institute Building, Room 319, 2 Anzhen Road, Chaoyang District, Beijing, 100029, China. fenglan@ccmu.edu.cn.

Abstract

Introduction: Spinal cord injury (SCI) is a neurological, medically incurable disorder. Human pluripotent stem cells (hPSCs) have the potential to generate neural stem/progenitor cells (NS/PCs), which hold promise in the treatment of SCI by transplantation. In our study, we aimed to establish a chemically defined culture system using serum-free medium and ascorbic acid (AA) to generate and expand long-term self-renewing neuroepithelial-like stem cells (lt-NES cells) differentiated from hPSCs effectively and stably.

Methods: We induced human embryonic stem cells (hESCs)/induced PSCs (iPSCs) to neurospheres using a newly established in vitro induction system. Moreover, lt-NES cells were derived from hESC/iPSC-neurospheres using two induction systems, i.e., conventional N2 medium with gelatin-coated plates (coated) and N2+AA medium without pre-coated plates (AA), and were characterized by reverse transcription polymerase chain reaction (RT-PCR) analysis and immunocytochemistry staining. Subsequently, lt-NES cells were induced to neurons. A microelectrode array (MEA) recording system was used to evaluate the functionality of the neurons differentiated from lt-NES cells. Finally, the mechanism underlying the induction of lt-NES cells by AA was explored through RNA-seq and the use of inhibitors.

Results: HESCs/iPSCs were efficiently induced to neurospheres using a newly established induction system in vitro. lt-NES cells derived from hESC/iPSC-neurospheres using the two induction systems (coated vs. AA) both expressed the neural pluripotency-associated genes PAX6, NESTIN, SOX1, and SOX2. After long-term cultivation, we found that they both exhibited long-term expansion for more than a dozen generations while maintaining neuropluripotency. Moreover, the lt-NES cells retained the ability to differentiate into general functional neurons that express β-tubulin at high levels. We also demonstrated that AA promotes the generation and long-term expansion of lt-NES cells by promoting collagen synthesis via the MEK-ERK1/2 pathway.

Conclusions: This new chemically defined culture system was stable and effective regarding the generation and culture of lt-NES cells induced from hESCs/iPSCs using serum-free medium combined with AA. The lt-NES cells induced under this culture system maintained their long-term expansion and neural pluripotency, with the potential to differentiate into functional neurons.

Keywords: Ascorbic acid; Human pluripotent stem cells; Long-term self-renewing neuroepithelial-like stem cells; Neurospheres; Spinal cord injury.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Ascorbic Acid / pharmacology
Cell Differentiation
Collagen
Embryonic Stem Cells
Humans
Induced Pluripotent Stem Cells*
Neural Stem Cells*

Substances

Collagen
Ascorbic Acid